Characterization of EVL-I as a protein kinase D substrate |
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| Authors: | Katrien Janssens Line De Kimpe Michele Balsamo Sandy Vandoninck Jackie R Vandenheede Frank Gertler Johan Van Lint |
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| Institution: | 1. Key Laboratory of South China Sea Fishery Resources Exploitation & Utilization of Ministry of Agriculture, Guangzhou 510300, China;2. South China Sea Resource Exploitation and Protection Collaborative Innovation Center (SCS-REPIC), Guangzhou 510300, China;3. South China Sea Fisheries Research Institute, Chinese Academy of Fishery Sciences, Guangzhou 510300, China;4. Key Laboratory of Marine Bio-resources Sustainable Utilization, Chinese Academy of Sciences, Guangzhou 510300, China |
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| Abstract: | EVL-I is a splice variant of EVL (Ena/VASP like protein), whose in vivo function and regulation are still poorly understood. We found that Protein Kinase D (PKD) interacts in vitro and in vivo with EVL-I and phosphorylates EVL-I in a 21 amino acid alternately-included insert in the EVH2 domain. Following knockdown of the capping protein CPβ and spreading on laminin, phosphorylated EVL-I can support filopodia formation and the phosphorylated EVL-I is localized at filopodial tips. Furthermore, we found that the lamellipodial localization of EVL-I is unaffected by phosphorylation, but that impairment of EVL-I phosphorylation is associated with ruffling of lamellipodia upon PDBu stimulation. Besides the lamellipodial and filopodial localization of phosphorylated EVL-I in fibroblasts, we determined that EVL-I is hyperphosphorylated and localized in the cell–cell contacts of certain breast cancer cells and mouse embryo keratinocytes. Taken together, our results show that phosphorylated EVL-I is present in lamellipodia, filopodia and cell–cell contacts and suggest the existence of signaling pathways that may affect EVL-I via phosphorylation of its EVH2 domain. |
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